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D6+TNF- α. D1+TNF- α. D6+DXR. D1+DXR. TNF- α. CTR. D1. D6. DXR. MW. 65 kDa. NF-kB. LAMIN. 65 kDa. Additional file 3 Figure S2 Effects of D1 and D6 on NFkB expression in neuroblastoma cell line. Legend
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D6+TNF-α D1+TNF-α D6+DXR D1+DXR TNF-α CTR D1 D6 DXR MW 65 kDa NF-kB LAMIN 65 kDa Additional file 3 Figure S2 Effects of D1 and D6 on NFkB expression in neuroblastoma cell line. Legend Effects of D1 and D6 on NFkB expression in neuroblastoma cells after treatments with either TNFa or Doxorubicin. SH-SY5Y were untreated (CTR) or treated with 3 mM of both D1 and D6 for 24 hours. Six hours before the end of the treatment, either 25 ng/ml TNFa or 2 mg/ml Doxorubicin (DXR) were added to the D1/D6 treated cells. Nuclear cellular fractions were processed by western blot analysis. Blot is representative of three independent experiments and data are normalized against Lamin A/C. Methods The human neuroblastoma cell line, SH-SY5Y, was grown in DMEM (Sigma). The cells were plated in 100 mm petri dishes, cultured for 24 hours and then untreated or treated with 3 mM of either D1 or D6 for 24 hours. Six hours before the end of the treatment, 25 ng/ml of TNFa (recombinant human TNFa, Strathmann-Biotec AG, Hamburg, Germany) or 2 mg/ml of Doxorubicin (Sigma) respectively, were added to the dishes. Nuclear cellular fractions were obtained and then processed by western blot analysis, as described in Material and Method. Lamin A/C was used as loading control.